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量化光合生物中蛋白质硫醇的可逆氧化

Quantifying reversible oxidation of protein thiols in photosynthetic organisms.

作者信息

Slade William O, Werth Emily G, McConnell Evan W, Alvarez Sophie, Hicks Leslie M

机构信息

Department of Chemistry, University of North Carolina at Chapel Hill, Chapel Hill, NC, 27599, USA.

出版信息

J Am Soc Mass Spectrom. 2015 Apr;26(4):631-40. doi: 10.1007/s13361-014-1073-y. Epub 2015 Feb 20.

DOI:10.1007/s13361-014-1073-y
PMID:25698223
Abstract

Photosynthetic organisms use dynamic post-translational modifications to survive and adapt, which include reversible oxidative modifications of protein thiols that regulate protein structure, function, and activity. Efforts to quantify thiol modifications on a global scale have relied upon peptide derivatization, typically using isobaric tags such as TMT, ICAT, or iTRAQ that are more expensive, less accurate, and provide less proteome coverage than label-free approaches--suggesting the need for improved experimental designs for studies requiring maximal coverage and precision. Herein, we present the coverage and precision of resin-assisted thiol enrichment coupled to label-free quantitation for the characterization of reversible oxidative modifications on protein thiols. Using C. reinhardtii and Arabidopsis as model systems for algae and plants, we quantified 3662 and 1641 unique cysteinyl peptides, respectively, with median coefficient of variation (CV) of 13% and 16%. Further, our method is extendable for the detection of protein abundance changes and stoichiometries of cysteine oxidation. Finally, we demonstrate proof-of-principle for our method, and reveal that exogenous hydrogen peroxide treatment regulates the C. reinhardtii redox proteome by increasing or decreasing the level of oxidation of 501 or 67 peptides, respectively. As protein activity and function is controlled by oxidative modifications on protein thiols, resin-assisted thiol enrichment coupled to label-free quantitation can reveal how intracellular and environmental stimuli affect plant survival and fitness through oxidative stress.

摘要

光合生物利用动态的翻译后修饰来生存和适应,这包括蛋白质硫醇的可逆氧化修饰,这些修饰可调节蛋白质的结构、功能和活性。在全球范围内对硫醇修饰进行定量的努力依赖于肽衍生化,通常使用等压标签,如TMT、ICAT或iTRAQ,这些标签比无标签方法更昂贵、准确性更低且蛋白质组覆盖范围更小,这表明对于需要最大覆盖范围和精度的研究,需要改进实验设计。在此,我们展示了树脂辅助硫醇富集与无标签定量相结合用于表征蛋白质硫醇可逆氧化修饰的覆盖范围和精度。以莱茵衣藻和拟南芥作为藻类和植物的模型系统,我们分别定量了3662个和1641个独特的半胱氨酰肽,变异系数(CV)中位数分别为13%和16%。此外,我们的方法可扩展用于检测蛋白质丰度变化和半胱氨酸氧化的化学计量。最后,我们证明了我们方法的原理,并揭示外源过氧化氢处理分别通过增加或减少501个或67个肽的氧化水平来调节莱茵衣藻的氧化还原蛋白质组。由于蛋白质的活性和功能受蛋白质硫醇氧化修饰的控制,树脂辅助硫醇富集与无标签定量相结合可以揭示细胞内和环境刺激如何通过氧化应激影响植物的生存和适应性。

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